1983～1992年中国陆地NDVI变化的气候因子驱动分析

利用1983－1992年NOAA／AVHRR逐月的归一化植被指数（NDVI）资料和中国国家气象局全国160个基本标准气象站的月均温和降雨数据,探讨气温,降水对中国植NDVI动态变化驱动作用。首先计算了NDVI与气温,降水偏相关和复相关系数,研究了中国植被NDVI变化的气候因子驱动的区域分异规律,并据此,对中国植被NDVI变化的气候因子驱动进行了分区,共分出4个一级区,6个二级区和14个三级区,进一步表明了中国植被NDVI变化气候因子驱动的区域差异。     

Physical mapping and microsynteny of Brassica rapa ssp. pekinensis genome corresponding to a 222 kbp gene-rich region of Arabidopsis chromosome 4 and partially duplicated on chromosome 5

We constructed a bacterial artificial chromosome (BAC) library, designated as KBrH, from high molecular weight genomic DNA of Brassica rapa ssp. pekinensis (Chinese cabbage). This library, which was constructed using HindIII-cleaved genomic DNA, consists of 56,592 clones with average insert size of 115 kbp. Using a partially duplicated DNA sequence of Arabidopsis, represented by 19 and 9 predicted genes on chromosome 4 and 5, respectively, and BAC clones from the KBrH library, we studied conservation and microsynteny corresponding to the Arabidopsis regions in B. rapa ssp. pekinensis. The BAC contigs assembled according to the Arabidopsis homoeologues revealed triplication and rearrangements in the Chinese cabbage. In general, collinearity of genes in the paralogous segments was maintained, but gene contents were highly variable with interstitial losses. We also used representative BAC clones, from the assembled contigs, as probes and hybridized them on mitotic (metaphase) and/or meiotic (leptotene/pachytene/metaphase I) chromosomes of Chinese cabbage using bicolor fluorescence in situ hybridization. The hybridization pattern physically identified the paralogous segments of the Arabidopsis homoeologues on B. rapa ssp. pekinensis chromosomes. The homoeologous segments corresponding to chromosome 4 of Arabidopsis were located on chromosomes 2, 8 and 7, whereas those of chromosome 5 were present on chromosomes 6, 1 and 4 of B. rapa ssp. pekinensis.     

两种除草剂对棉田节肢动物群落多样性指数的影响

系统地研究了棉田地面和棉株节肢动物群落及各亚群落施用克无踪(A)、高盖(B)与对照(CK)之间在群落生物多样性、丰富度和均匀度的差异.结果表明,对地面肉食动物群落生物多样性(H′)的A-CK的t值为3.099,B-CK的t值为2.449,t＞t_0.05=2.228,差异显著;地面植食动物亚群落的(H′)A-CK的t值为2.377,A-B为2.260,t＞t_0.05=2.228,差异均显著.棉株节肢动物群落及亚群落A-CK、B-CK和A-B之间差异不显著.地面节肢动物亚群落丰富度A-CK的t值为4.759,地面植食类节肢动物亚群落为4.359,地面肉食节肢动物亚群落为2.963,均t＞t0.0=2.228,表明A与CK之间差异显著;在均匀度上,A和B及A-CK、B与CK之间两类群落及亚群落上差异均不显著.A和B对棉株节肢动物群落影响很小.施用A和B及CK的生物多样性的变化总趋势一致.     

Growth of Pichia guilliermondii A9, an osmotolerant yeast, in waste brine generated from kimchi production

The possibility of culturing an osmotolerant yeast using waste brine from a kimchi factory as a substrate for the production of single cell protein was investigated. Pichia guilliermondii A9 was selected from 70 isolates of yeast demonstrating substantial growth in the waste brine. The growth of P. guilliermondii A9 in waste brine was not inhibited by NaCl concentrations of up to 10% (w/v). However, it was reduced drastically at concentrations greater than 12% (w/v). Approximately 90% of BOD was removed from the waste brine by culturing of P. guilliermondii A9 for 24 h. The maximum cell yield was 0.69 g of dry cells per liter, containing 40% of protein. When the waste brine was enriched with cabbage juice from waste cabbage, the final cell mass increased proportionally with the amount of added organic material. Salt stressed cells of P. guilliermondii A9 grown in waste brine are shown in scanning electron micrographs. In conclusion, the large amounts of waste brine generated from kimchi production could be used directly for the culture of the osmotolerant yeast P. guilliermondii A9.     

贵州地方山羊品种的RAPD分析

用180条引物对黔东南小香羊、贵州白山羊、贵州黑山羊和黔北麻羊4个贵州地方山羊品种(种群),以及南江黄羊和波尔山羊进行RAPD分析,其中27条引物扩增出多态性图谱。这27条引物共扩增出281条带,多态带为115条,平均多态频率为40．92％(范围20％～80％);每条引物平均扩增条带为10．41条(范围4～16条);扩增带分子量在210～2800bp。贵州白山羊与贵州黑山羊之间的遗传距离指数(0．0605)最小,而波尔山羊与其他品种之间的遗传距离指数(0．1059～0．1488)最大。NJ法聚类结果显示,贵州白山羊与贵州黑山羊间的亲缘关系最近,其次为黔北麻羊,而黔东南小香羊与其他3个贵州地方品种的亲缘关系较南江黄羊还远。分析表明,黔东南小香羊在遗传上为一独立的品种;而贵州地方山羊品种间具有较近的亲缘关系,遗传变异较小,具有较高的遗传稳定性。     

家蚕抗菌肽在毕赤酵母中的表达

目的：用毕赤酵母真核系统表达有抑菌活性的家蚕抗菌肽(cecropin-XJ)。将pGEX-4T-1-cecropin-XJ上的抗菌肽基因cecropin—XJ克隆至穿梭质粒pSuperY上,用Bln Ⅰ酶切使之线性化后,采用电击法转化酵母SMD1168,转化子用小瓶发酵,经SDS—PAGE检测,表达产物可以在α信号因子的引导下,分泌到培养基中,且表达产物具有明显抑菌活性。     

Design, synthesis, and biological evaluation of novel 4-alkylamino-1-hydroxymethylimidazo[1,2-a]quinoxalines as adenosine A(1) receptor antagonists

A series of 4-alkylamino-1-hydroxymethylimidazo[1,2-a]quinoxalines have been synthesized and evaluated for their adenosine A(1) receptor inhibitory activity in the radioligand binding assays. The compounds were tested for the inhibition percent (IP) and the affinity toward A(1)AR (K(i)) that IP were more than 90% in the nanomolar range. 4-Cyclopentylamino-7,8-dichloro-1-hydroxymethylimidazo[1,2-a]quinoxaline 18 is the most potent compound in this series, having K(i)=7nM, which is remarkably higher than that of IRFI-165 (K(i)=48). 1-Hydroxymethyl groups of the tricyclic heteroarmatic compounds displayed the potent affinities toward A(1)AR.     

用生物信息学方法寻找肝癌特异性表达基因转录调控模式

为了对肝癌(hepatocellularcarcinoma,HCC)的分子发病机理进行研究,首先对肝癌基因表达谱数据用t-检验算法进行了分析,找到了肝癌中特异性表达基因(characteristicgenes).然后把这些基因结合已知的肝HNF家族转录因子染色质免疫共沉淀结合DNA启动子芯片(ChIP-chip)实验数据用SAEM算法进行分析,得到了肝癌特异性表达基因的转录调控关系,并寻找到了多个HNF家族转录因子调控单基因的转录调控模式.结果表明HNF家族转录因子对大量具有重要功能的肝癌特异性表达基因进行了转录调控,并且多个HNF家族转录因子调控单基因可以形成前馈环和多输入调控等模式.     

红色荧光蛋白在丝状真菌里氏木霉中的表达

目的:建立红色荧光蛋白在里氏木霉中的表达方法,为深入研究里氏木霉中纤维素酶的合成机理打下基础。方法:采用PCR方法分离了里氏木霉纤维二糖水解酶Ⅰ(CBHⅠ)的启动子(Pcbh1)和终止序列(Tcbh1),将这两个片段与红色荧光蛋白(DsRed)的基因连接,得到Pcbh1-DsRed-Tcbh1表达盒。用此表达盒和质粒pAN7-1对里氏木霉QM9414的原生质体进行共转化,并用含100μg/ml潮霉素B的选择性平板进行筛选。结果:经筛选得到20个抗性转化子,在乳糖的诱导下有5个转化子可以表达红色荧光蛋白。对插入片段进行了扩增和序列测定,结果表明DsRed通过同源重组整合到了转化子的基因组DNA上,并处于cbh1启动子的下游。结论:通过cbh1启动子可以实现红色荧光蛋白在里氏木霉细胞内的稳定表达。